coatings Development of Antibacterial, Antioxidant, and UV-Barrier Chitosan Film Incorporated with Piper betle Linn Oil as Active Biodegradable Packaging Material

: This study aims to introduce the antibacterial and antioxidant activities of the Piper betle Linn oil (PBLO) into chitosan ﬁlm (pCS), named as pCS-PBLO ﬁlm. The morphology, structure, and properties of the pCS-PBLO ﬁlm, along with the PBLO concentration between 0.4% and 1.2% ( v / v ), were determined. The ﬁlm surface became rough and heterogeneous with the addition of PBLO, which directly inﬂuenced on mechanical strength of the resultant ﬁlm. The addition of the PBLO did not affect thermal stability but signiﬁcant effect on ﬂexibility and mobility of the ﬁlm. Importantly, the ﬁlm enhanced the UV-protective property and antioxidant activity as incorporated-PBLO. Moreover, the resulting ﬁlm revealed the great inhibition efﬁciency against the negative-gram ( E. coli , P. aeruginosa , and S. typhi ) and positive-gram ( S. aureus ) bacteria based on phenolic compounds, such as the acetyleugenol, eugenol, 4-allyl-1,2-diacetoxybenzen, and chavicol acetate in PBLO components. In particular, the pCS-PBLO ﬁlm may extend the shelf life of king oranges up to two weeks at 25 ◦ C that is longer as compared to the uncoated sample and coated with chitosan alone. These results suggest that the pCS-PBLO ﬁlm can be used as environmental-friendly and effective food packaging material in the future.


Introduction
Petroleum-based plastics are one of the main contributors to serious environmental pollution due to their un-degradable characters. It was found that thousands of marine property of resultant film as compared to the addition of PBLLE because of high hydrophobicity of PBLO. Interestingly, the light of present work was high transparent of film made from chitosan and PBLO in visible region as compared to chitosan film containing PBLLE in dark brownish which significantly affected to see-through property important for food packaging material as customer want to see packaged product before buying. Bedsides to this, the combination of nontoxic components including chitosan and Piper betel Linn oil is considered to be safe material for food packaging.

Analyses of PBLO
Chemical composition of PBLO was determined by using GC Agilent 6890N instrument (California, CA, USA) equipped with MS 5973 inert and HP5-MS column. The head column pressure was 9.3 psi and helium worked as the carrier gas with velocity of 1 mL/min. Before testing, 25 µL of PBLO was mixed in 1 mL of n-hexane and further dehydrated by Na 2 SO 4 . The injection temperature was set at 250 • C and split injection in the ratio of 1:100. Thermal profiles were set up as follows: the initial column temperature at 50 • C for 2 min, continued up to 80 • C at velocity of 2 • C/min, continually increasing to 150 • C at velocity of 5 • C/min, and followed to increase to 300 • C at velocity of 20 • C/min for 5 min. The individual compound was identified and confirmed by comparing to those of available library data from GC/MS system.

Preparation of pCS-PBLO films
Chitosan solution was produced by dissolving 1 g of chitosan powder in 100 mL of aqueous acetic acidic solution (1%, v/v). The solution was magnetically stirred at 800 rpm and room temperature (at around 27 • C) for 24 h to dissolve completely solids. Glycerol (30%, w/w) was then added into chitosan solution with the function of plasticizer. Subsequently, the PBLO was added into plasticized chitosan solution at different volume ratio [0.4%, 1%, and 1.2% (v/v)] before adding 0.2% (w/v) of Tween 80 as an emulsifier. Finally, film-forming solution was casted on the 20 cm × 20 cm plastic mold and further dried at 40 • C for 48 h. After drying, the chitosan-based blend films were peeled off and kept at 25 • C for further analyses. The control chitosan film was denoted as pCS and chitosan films containing PBLO were remarked as pCS-0.4PBLO, pCS-1PBLO, and pCS-1.2PBLO with respect to incorporated PBLO content at 0.4%, 1%, and 1.2% (v/v). The thickness of films was controlled by taking equal volume in film fabrication process to ensure ignorable variation and thickness values were recorded at 0.053 ± 0.002; 0.055 ± 0.003; 0.064 ± 0.003; and 0.078 ± 0.004, respectively for pCS, pCS-0.4PBLO, pCS-1PBLO, and pCS-1.2PBLO.

Film Characterization
The surface morphology of the as-prepared films was recorded using scanning electron microscope (SEM) on JSM-IT200 equipment (Massachusetts, MA, USA). The attenuated total reflection (ATR)/Fourier transform infrared (FTIR) (ATR/FTIR) spectra of the as-prepared films were determined using a JASCO FT/IR-6600 instrument (JASCO International Co., Tokyo, Japan) in the wavenumber ranged from 4000-500 cm −1 . The thermo-stability of the as-prepared films was determined using the thermogravimetric analyses (TGA) and derivative thermogravimetric (DTG) on a TGA model Q500 V20.10 Build 36 (TA Instruments, Hüllhorst, Germany) by a temperature program of 27-800 • C with heating rate of 10 • C/min. The crystal structure of the as-prepared films was determined using X-ray diffraction (XRD) on a Bruker D8 Advance powder diffractometer (Bruker AXS GmbH, Berlin, Germany) with Cu-Kα radiation source and 2θ range of 2-60 • with 0.2 s/step. The mechanical behavior of the as-prepared films was measure on AG-Xplus Series Precision Universal Testers following to ASTM-D882 standard [24] with the size film of 15 mm × 100 mm and gauge length of 50 mm and crosshead speed of 10 mm/min at room temperature (at around 27 • C). The transmittance of the as-prepared films was recorded on UV-1800 UV/Visible Scanning Spectrophotometer (Shimadzu Scientific Instruments Inc., Kyoto, Japan) in wavelength range of 190-800 nm.
Swelling degree (SD) was performed based on the method previously described [25]. Five pieces (2 cm × 2 cm) of film were initially dried at 70 • C for 24 h and weighted to get dry weight denoted as m 1 . Then, the dried pieces of film were soaked in 30 mL of distilled water for 24 h at room temperature (27 • C). For next step, the pieces of film were separated from water and removed the residual surface water using tissue paper and further weighted (m 2 ). The SD (%) was calculated by following equations:

Bacterial Inhibition Test
The antibacterial activities of the pCS and pCS-PBLO films were tested using the agar diffusion and liquid incubation methods as previously descriptions [25,26]. For the agar diffusion tests, a 100 µL (an approximately titer of 2 × 10 6 colony forming units per mL, CFU/mL) of each bacterial strain, including the S. aureus, S. typhimurium, E. coli, and P. aeruginosa, was spread onto the LB agar plates (Sigma-Aldrich, Missouri, MO, USA) in triplicate. A 1-cm 2 slide of each pCS and pCS-PBLO films were then added onto midpoint of the plates (Supplementary Figure S1). Subsequently, the plates were incubated at 37 • C for 24 h. The inhibition zone diameters were measured with a ruler.
For the liquid incubation tests, only the E. coli strain was used. A 2-cm 2 slide of each pCS and pCS-PBLO films was added into the tubes containing 2 mL of the LB medium. The 5% (v/v) of bacterial suspension at density of 2 × 10 8 CFU/mL was added into the tubes. The tubes were incubated in sharking incubator at 37 • C and 200 rpm. The medium was collected at different incubated times of 0, 4, 8, 11, and 24 h, and direct spread onto the agar plates in triplicate to evaluate the bacterial viability.
(where: A, total colonies in 1 mL of sample; N, total colonies in three agar plates; and f, the dilution factor).

Antioxidant Test
The antioxidant activity of chitosan solution with and without PBLO was determined using 2,2-diphenyl-1-picrylhydrazyl free radical (DPPH·) method previously described by Brand-Williams et al. [27]. Initially, the chitosan-PBLO solutions were diluted in distillated water to obtain the different concentration seri (500-32.25 µg/mL). The diluted sample solution (1 mL) was added into 1 mL of 0.3 mM DPPH· methanol solution and further well-vortexed for 7 s before dark-incubating for 60 min at ambient temperature (27 • C). After dark-incubated, the UV-Vis absorbance of mixture solution was measured at 517 nm. The scavenge efficiency to DPPH free radical was calculated in the following equation: (where OD c and OD t are respectively the absorbance of 0.3 mM DPPH· methanol solution and the chitosan-PBLO solution). Antioxidant activity of PBLO containing chitosan film was evaluated through IC 50 (µg/mL) which was determined from the plot of working sample concentration versus SE%. The experiments were replicated in triplicates to get an average IC 50 parameter for each composition.

Surface Tension, Work of Adhension, and Spreading Coefficient
The coating efficiency of the coating solution was evaluated by the work of adhesion and spreading coefficient due to contact angle measurement of coating liquids over orange skin [28]. Surface tension of coating solution and contact angle of all chitosan solution with and without PBLO over orange skin was determined by using a Theta Optical Goniometer (Jersey, NJ, USA). The adhesion and spreading coefficient were calculated according to the Wenzel equation [29] as follows: Spreading coe f f icient = γ 1 (cos θ − 1) where γ 1 and θ are respectively the surface tension of coting solution and the contact angle of the film coating on the orange skin.

Coating of King Oranges
King oranges were pre-treated by washing with distilled water and further blow-dried under a fan at ambient temperature (27 • C). The king oranges were coated by chitosan and chitosan-PBLO solution using the pressure-spraying method. The uncoated oranges were used as control sample. All coated samples were then stored at 25 • C and daily evaluated the appearance changes for 2 weeks.

ATR/FTIR Analyses
ATR/FTIR spectroscopy was used for the purpose of identifying chemical functional groups and determining possible interaction between components in polymeric blend. The spectrum of film made from chitosan alone presents an absorption band in the range of 3624-3012 cm −1 due to the overlapping of O-H and N-H stretching vibration ( Figure 1) [32]. The C-H antisymmetric and symmetric stretching vibrations of -CH 2 groups were recorded at 2873 cm −1 [33]. The characteristic chitosan signs were observed at 1650 cm −1 belonging to C=O stretching vibration in amide-I, 1532 cm −1 corresponding to C-N stretching vibration composed in amide-II and N-H bending vibration, and 1400 cm −1 (HN-CO stretching vibration in amide-III) [32,34]. Meanwhile the sharp peak at 1020 cm −1 was related to C-O stretching vibration [34]. It was found that appreciable changes in chitosan ATR-FTIR spectrum by the addition of PBLO. For instance, the absorption band at 3624-3012 cm −1 (O-H and N-H stretching vibration) became weaker and more flatted by the addition of PBLO. The decrease in the peak intensity at 1533 cm −1 corresponding to C-N stretching vibration and 1402 cm −1 (NH-CO stretching vibration) by the addition of PBLO along with the significant evolution of shoulder at 1584 cm −1 due to the aromatic ring vibration of phenolic compounds [33]. Furthermore, the absorption band at 1020 cm −1 (corresponding to C-O stretching vibration) in the film formulation made from chitosan and PBLO shifted to higher frequency region and became more intense and compared to those in control chitosan spectrum when PBLO abundantly contained C-O groups in structure of phenolic compounds. These changes were likely ascribed to the hydrogen-bonding interaction between O-H and N-H groups in chitosan and hydroxyl of phenolic compound in PBLO [33]. Murat Kaya et al. [33] also found the possible hydrogen interactions arising between film functional groups and Berberis crataegina s seed oil evidenced by the slight shift in the C-O stretching vibration peak to a higher frequency region when seed oil was incorporated into chitosan.
bonding interaction between O ̶ H and N ̶ H groups in c compound in PBLO [32]. Murat Kaya et al. [34] als interactions arising between film functional groups a evidenced by the slight shift in the C ̶ O stretching vibr region when seed oil was incorporated into chitosan.
The ATR/FTIR results indicated the existence of int functional groups in PBLO and chitosan, which could b into environment and thus allowing maintaining antiba blend films during food protection.

XRD analyses
Possible structural changes in chitosan network w confirmed by XRD ( Figure 2). The film made from chi peaks at 11.4° and 18.1°, which are closely related to anh [7,35], and a typical fingerprint at 20.8° attributed to am The disappearance of crystal peaks at 11.4° and 18.1° intensity at 20.8° as the addition of 0.4% (v/v) and 1.2% crystallinity of blend film. It is likely suggested that int phenolic groups in PBLO and chitosan functional gr molecular interaction between chitosan chains resu amorphous region [33]. Besides to this, the new pr identified at 14.4° with 1.2% (v/v) PBLO addition, pro The ATR/FTIR results indicated the existence of inter-molecular interaction between functional groups in PBLO and chitosan, which could be expected to diminish oil release into environment and thus allowing maintaining antibacterial and antioxidant activity of blend films during food protection.

XRD Analyses
Possible structural changes in chitosan network with the addition of PBLO were confirmed by XRD ( Figure 2). The film made from chitosan alone reveals characteristic peaks at 11.4 • and 18.1 • , which are closely related to anhydrous and hydrated crystalline [7,35], and a typical fingerprint at 20.8 • attributed to amorphous state of chitosan [36,37]. The disappearance of crystal peaks at 11.4 • and 18.1 • and the increase in diffraction intensity at 20.8 • as the addition of 0.4% (v/v) and 1.2% (v/v) PBLO imply a decrease in crystallinity of blend film. It is likely suggested that inter-molecular interaction between phenolic groups in PBLO and chitosan functional groups hinder and disturb intra-molecular interaction between chitosan chains resulting in the predominance of amorphous region [34]. Besides to this, the new pronounced diffraction peak was identified at 14.4 • with 1.2% (v/v) PBLO addition, probably indicating that such inter-molecular interactions exert the rearrangement in polymeric network to generate newly ordered structure. The similar behavior in the reduction in crystalline was documented in chitosan consisted of polyphenols from thinned young apple [37]. However, re-evolution of the crystalline peaks at 11.4 • and 18.1 • with higher diffraction intensity in chitosan film containing 1% (v/v) PBLO is still unclear, it is likely to suggest that the position of original ordered chains in control chitosan are replaced by a large amount of crosslinking network between chitosan and PBLO. It can be therefore concluded that the addition of PBLO may convert semi-crystalline in chitosan film toward more amorphous structure, which significant affect to mechanical behavior of the blend film in further investigation.
11.4° and 18.1° with higher diffraction intensity in chitos is still unclear, it is likely to suggest that the position of chitosan are replaced by a large amount of crosslinkin PBLO. It can be therefore concluded that the addition o line in chitosan film toward more amorphous structur chanical behavior of the blend film in further investigat

Thermo-Stability
TGA and DTG analyses were utilized for the purpos of film made from chitosan alone and containing PBLO. A the control chitosan film presents three-stage decompos was due to the vaporization of adsorbed water on the fil acetic acid (80-150 °C) [19,38]. The decomposition of gl at 150-250 °C [19]. The main degradation stage at 250-3 S1) was attributed to the saccharide ring dehydration an bone [19]. In case of chitosan with PBLO, there are th documented at 50-150 °C, 150-360 °C, and 360-450 °C. composition of glycerol is negligible in the TGA curves composition stage not found in chitosan alone appears position of aromatic compounds in PBLO and surfact thermal behavior of chitosan film with and without PB from DTG profile. In details, the decomposition peak of at 296 °C and 284 °C for control chitosan and pCS-PB

Thermo-Stability
TGA and DTG analyses were utilized for the purpose of investing the thermal stability of film made from chitosan alone and containing PBLO. As seen in TGA curves (Figure 3a), the control chitosan film presents three-stage decomposition. The first stage at 50-150 • C was due to the vaporization of adsorbed water on the film surface (50-80 • C) and residual acetic acid (80-150 • C) [19,38]. The decomposition of glycerol-based plasticizer occurred at 150-250 • C [19]. The main degradation stage at 250-360 • C with 43% weight loss (Table S1) was attributed to the saccharide ring dehydration and decomposition of chitosan backbone [19]. In case of chitosan with PBLO, there are three steps of decomposition were documented at 50-150 • C, 150-360 • C, and 360-450 • C. It should be noticed that the decomposition of glycerol is negligible in the TGA curves of blend films and the newly decomposition stage not found in chitosan alone appears at 400-450 • C due to the decomposition of aromatic compounds in PBLO and surfactants [34,38,39]. The difference in thermal behavior of chitosan film with and without PBLO was pronouncedly observed from DTG profile. In details, the decomposition peak of chitosan backbone was recorded at 296 • C and 284 • C for control chitosan and pCS-PBLO film, respectively. This result indicated that the thermal stability of chitosan film slightly decreased by the addition of PBLO. More interesting, it was not found the PBLO own degradation peak. This was likely pointed that PBLO was well-embedded in blend film due to the inter-molecular interaction between phenolic compounds and chitosan functional groups resulting in good protective effect and preventing separate decomposition of PBLO.

The Surface Morphology
The surface images at micro level of film formulation made containing 0.4-1.2 % (v/v) PBLO are observed in Figure 4. Herei ally used as plasticizer for all the films and the successful film formulations was obtained as expected. The control chitosan played uniform, smooth, homogeneous appearance without crac ing compact and continuous structure. Meanwhile the film mad and PBLO presented the rough and heterogeneous surface with ical-like droplets, resulting in discontinuities in blend film that m

The Surface Morphology
The surface images at micro level of film formulation made from chitosan alone and containing 0.4-1.2 % (v/v) PBLO are observed in Figure 4. Herein, glycerol was additionally used as plasticizer for all the films and the successful film formation for all applied formulations was obtained as expected. The control chitosan film without PBLO displayed uniform, smooth, homogeneous appearance without cracks and fractures, indicating compact and continuous structure. Meanwhile the film made from blend of chitosan and PBLO presented the rough and heterogeneous surface with the appearance of spherical-like droplets, resulting in discontinuities in blend film that may affect to weak fracture resistance of film. The existence of spherical-like droplets indicated the dispersion of lipid droplets on the surface of resulting films. However, the spherical-like droplets were not found on the surface of chitosan film incorporated with Piper betle Linn leaf extract [23,40]. Similar findings were found in chitosan film containing 0.4-1.2% (w/v) Origanum vulgare L. oil [30], and 1-4% (v/v) Eucalyptus globulus oil [20], when spherical oil droplets tended to separate and center at the upper surface of film, likely resulted from the traction force caused by chitosan matrix during drying step. At lower PBLO content (0.4%, v/v), lipid droplets were scarcely observable since they abundantly concentrated on the surface of film with small droplet size. As increasing PBLO concentration to 1% (v/v), droplet size slightly enlarged and became visible. However, the film surface became more heterogeneous when some spherical-like droplets were embedded and trapped in the polymeric network. The slight increase in droplet size may due to the fact that flocculation and coalescence occurred at higher lipid content [41]. Although droplet size of lipids was lower, the surface of chitosan film containing 1.2% (v/v) PBLO become more homogeneous as compared to that in inclusion of 0.4% (v/v) and 1% (v/v) PBLO. The decrease in lipid size likely due to well-embedded oil droplets in polysaccharide matrix resulting in the change in the shape of lipid droplets. This observation was coincident with what was seen gelatin-chitosan containing Origanum vulgare L. essential oil (OEO) as higher droplet size was found in film incorporated with 0.8%(w/v) OEO than that in 0.4 (w/v) and 1.2 (w/v) incorporated-OEO [42].

UV-Protective Property
The high transparent and see-through property are important for food packaging material because it easily attract customer who want to see packaged product before buying. The UV barrier property is of great benefit to protect food preventing photo-oxidation and degradation of vitamin and other photosensitizers [43]. The light transmittance in UV-Vis of 200-800 nm for chitosan-based films is displayed in Figure 5. The film made from chitosan alone presents low transmittance in the UVC region (250-280 nm) on the ground of the existence of double bond (CO) in remaining chitin after the deacetylation [44]. It was also found that about 90% light in visible region (400-800 nm) transmitted though control chitosan film meanwhile the chitosan incorporated with 0.4-1.2% (v/v) PBLO presented the light transmittance of 70% in this band. Interestingly, the light transmittance of film formulation made from chitosan containing 0.4% (v/v) and 1% (v/v) PBLO was near zero in the region of UVC (250-280 nm) and UVB (280-320 nm) and enlarged to UVA (320-400 nm) with 1.2% (v/v) incorporated-PBLO. This is due to UV absorbance of phenolic compounds bearing hydroxyl groups conjugated aromatic rings. Similar behavior was also documented as combining chitosan and turmeric extract (mainly composed curcuminoids) which acted as UV absorber due to aromatic groups in the curcuminoids [6]. It can be therefore concluded that film made from chitosan and PBLO can completely block the UV light without significantly reducing the see-through character of food packaging material, which was improved as compared to chitosan film incorporated with Piper betle Linn leaf extract in our previous report [23].

UV-Protective Property
The high transparent and see-through property are important for food packaging material because it easily attract customer who want to see packaged product before buying. The UV barrier property is of great benefit to protect food preventing photo-oxidation and degradation of vitamin and other photosensitizers [43]. The light transmittance in UV-Vis of 200-800 nm for chitosan-based films is displayed in Figure 5. The film made from chitosan alone presents low transmittance in the UVC region (250-280 nm) on the ground of the existence of double bond (C=O) in remaining chitin after the deacetylation [44]. It was also found that about 90% light in visible region (400-800 nm) transmitted though control chitosan film meanwhile the chitosan incorporated with 0.4-1.2% (v/v) PBLO presented the light transmittance of 70% in this band. Interestingly, the light transmittance of film formulation made from chitosan containing 0.4% (v/v) and 1% (v/v) PBLO was near zero in the region of UVC (250-280 nm) and UVB (280-320 nm) and enlarged to UVA (320-400 nm) with 1.2% (v/v) incorporated-PBLO. This is due to UV absorbance of phenolic compounds bearing hydroxyl groups conjugated aromatic rings. Similar behavior was also documented as combining chitosan and turmeric extract (mainly composed curcuminoids) which acted as UV absorber due to aromatic groups in the curcuminoids [6]. It can be therefore concluded that film made from chitosan and PBLO can completely block the UV light without significantly reducing the see-through character of food packaging material, which was improved as compared to chitosan film incorporated with Piper betle Linn leaf extract in our previous report [23]. block the UV light without significantly reducing the se aging material, which was improved as compared to chi betle Linn leaf extract in our previous report [23].

Mechanical Behavior
Sufficient mechanical property of edible films makes an important contribution to protect the integrity of packaging materials during storage and transportation. The tensile strength (Ts), elongation at break (Eb), and elastic modulus (Em) of chitosan-based blend films were recorded at 15.26 MPa, 17.49%, and 111.96 MPa, respectively ( Table 1). The incorporated-PBLO caused a considerable decrease in Ts (15.26-5.42 MPa) and Em (111.96-25.95 MPa). This behavior is likely due to the presence of oil droplets as observed in SEM images, hindering and interfering chain-chain interaction in chitosan resulting in discontinuities in polymeric chains and thus allowing decreasing fracture resistance and stiff of blend film. Furthermore, the weak inter-molecular interaction between chitosan and PBLO which may partially alter powerful chain-chain interactions [45]. Notably, the film made from chitosan and PBLO became more flexible and mobile evidenced by increasing elongation at break (17-25%) compared to the film without PBLO. This behavior was partially due to the presences of lipid droplets in film matrix which hinder polymer chain-chain interaction and result in flexible domains in film [46]. Furthermore, phenolic components interacted with chitosan functional groups and weaken the intra molecular forces among polymeric chains resulting in the increment in mobility and flexibility of chitosan film [45]. Another possible explanation due to the presence of emulsifier like Tween 80, importantly contributed to plasticizing effect as synergistic effect between glycerol surfactants with small molecules which could stay between polymeric chains and increase the chain mobility [47]. It was found that the film containing chitosan and PBLO offered more flexibility and mobility in comparison with chitosan/Piper betle Linn extract [23]. Similar findings were reported based on the addition of thyme and clove essential oil into chitosan film [48] and Origanum vulgare L. essential oil into gelatin-chitosan [42] that induced a reduction in Ts although a significant increase in Eb was observed. In contrast, the film made from chitosan incorporated cinnamon essential oil [16], and Apricot (Prunus armeniaca) kernel essential oil [22] presented an increase in Ts and decrease in Eb compared to chitosan alone. Whereas other essential oils such as Perilla frutescens (L.) Britt. essential oil [19], basil essential oil [18], Zataria multiflora Boiss essential oil [17] caused a significant reduction in both Ts and Eb. These differences as essential oils were added into simple chitosan film [17][18][19] on mechanical behavior may be mainly due to different kinds and components contained in essential oil, testing conditions as well as emulsifying agents [19].
In general, the addition of PBLO into chitosan resulted in more flexible and mobile blend films as merit for food packaging material.

Swelling Degree
The swelling index is a crucial parameter because it is closely related to the integrity of food packaging materials in water media. The swelling progress of chitosan film is due to hydrophilic amino groups which interact with water molecules via hydrogen bonding. Then, the diffusion of water into polymeric matrix resulting making polymer chain relaxed and hydrated therefore leading to expansion in whole polymer network before degradation [49,50]. The degree of swelling of control chitosan film after 24 h immersed in water was recorded at 50% ( Table 2). All PBLO incorporated chitosan films show higher swelling degree compared to control chitosan. This result is coincided with XRD analyses as the addition of PBLO may convert semi-crystalline in chitosan film toward more amorphous structure. Therefore, the swelling index increased progressively as the incorporated PBLO content augmented. This is opposite with chitosan film incorporated with Piper betle Linn leaf extract in our previous report [23]. The uptrend was likely due to the formation of chemical interaction between functional groups (-OH, -NH 2 ) of chitosan and high molecular phenolic groups in PBLO that exerts the partial disruption in polymeric network during 24 h swelling test [17].

Antibacterial Activity
The antibacterial activities of films were tested by using agar diffusion and liquid incubation methods [25,26]. The bacterial viability levels were evaluated using the inhibition diameters of ≥28 mm, 16-28 mm, 12-16 mm, and ≤12 mm for the strong, moderate, mild, and no activities, respectively [51]. As shown in Figure 6, the pCS-PBLO films were evaluated as moderate activities against the E. coli, P. aeruginosa, and S. typhi, except the S. aureus, in which the S. typhi was most vulnerable. In addition, the inhibition activity significantly increased in accordance with the increase of the PBLO from 0.4% to 1% (v/v). However, the PBLO at concentration of 1.2% (v/v) did not reveal further increased inhibition efficiency. In contrast, no inhibition zone was observed with the control pCS ( Figure S1). This result is accordance with previous reports that the antibacterial activity of chitosan in solid form was negligible because only bacteria directly exposing with active sites were inhibited [16,42]. Similar finding showed that the eugenol, mainly consisted in PBLO, may disrupt the cytoplasmic membrane of S. typhi and rise the permeability in bacterial cell [52]. The cell death was resulted from the ion leakage and loss of intracellular proteins. The compactness in polymeric network of pCS-PBLO film may hinder the exposure between bacterial cells and phenolic molecular [16,53].
disrupt the cytoplasmic membrane of S. typhi and rise the perm [52]. The cell death was resulted from the ion leakage and loss o The compactness in polymeric network of pCS-PBLO film may h tween bacterial cells and phenolic molecular [16,53]. Liquid inoculation tests showed that inhibition activities of the p was observed at all tested-PBLO concentrations of 0.4%, 1%, and 1 However, at low PBLO concentration of 0.4%, the number of bac of co-inoculation. Interestingly, at PBLO concentration of 1.2%, ba 24 h of co-inoculation. It found that the antibacterial activity of C than film containing Piper betle Linn extract [23], which was due volatile phenolic compound during oil preparation process. In g PBLO significantly improved the antibacterial activity of control sults indicated that the PBLO can be used as an antibacterial agent tive food packaging film products. Liquid inoculation tests showed that inhibition activities of the pCS-PBLO to E. coli strain was observed at all tested-PBLO concentrations of 0.4%, 1%, and 1.2% (Table 3, Figure S2). However, at low PBLO concentration of 0.4%, the number of bacteria increased after 8 h of co-inoculation. Interestingly, at PBLO concentration of 1.2%, bacteria were killed after 24 h of co-inoculation. It found that the antibacterial activity of CS-PBLO film was lower than film containing Piper betle Linn extract [23], which was due to the composition of volatile phenolic compound during oil preparation process. In general, the addition of PBLO significantly improved the antibacterial activity of control chitosan film. These results indicated that the PBLO can be used as an antibacterial agent in producing the effective food packaging film products.

Antioxidant Activity
In addition to bactericidal activity, PBLO as an antioxidant source incorporated with chitosan film may scavenge the free radicals preventing the oxidation of nutritional components and food deterioration. The antioxidant activity of pCS-PBLO films was evaluated through the half maximal inhibitory concentration (IC 50 ) which was determined as the concentration of sample required to scavenge 50% of DPPH radicals. The lower the IC 50 value is, the stronger the antioxidant activity is. Herein, IC 50 values of films containing 0.4, 1.0, and 1.2% (v/v) PBLO were resulted in 48.43, 44.86, and 42.49 µg/mL, indicating that antioxidant activity of resultant films increased with increasing incorporated PBLO concentration. The phenolic compound bearing -OH groups in PBLO may contribute to antioxidant mechanism as they scavenge DPPH· by donating either electron or hydrogen radical to free radical [54]. The IC 50 index was not documented for control chitosan film. Although active amino groups presenting in chitosan structure can react with free radical, the inhibitory efficiency of neat chitosan to DPPH was lower than 50% [55]. It can be observed the antioxidant activity of chitosan film was improved by the incorporation of PBLO; however, this property was lower as compared to that in the film containing Piper betle Linn extract [23]. These results revealed that PBLO containing chitosan films hold great antibacterial and antioxidant activities making them ideally suitable for food packaging film.

Preservative Application
The king orange, a variety of citrus fruit from Vietnam, was chosen for the test because it abundantly contained high nutritional values, especially rich in vitamin C. The appearance of king oranges with and without chitosan-based coatings, stored at 25 • C for 2 weeks were showed (Figure 7). The uncoated samples (control) were utilized to compare with coated king oranges. The bright green rind is observed for control sample while coated oranges reveals shinier and bright green rind surface on the first day. However, the rind of control sample moved to light yellow in color after storage 5 days but those do not occur for coated oranges. After 10 days, the bright yellow color is clearly viewed in control and chitosan coating on the orange surface begins to peel off. Interestingly, pCS-0.4PBLO coated orange still keep bright green and shiny skin after 10 days and up to two weeks. This is supported by the fact that higher work of adhesion and spreading coefficient of pCS-0.4PBLO solution over orange skin as compared to chitosan based coating liquids (Table S2). For cross-section images, the dense and compact texture are obviously observed for the king orange coated by chitosan and chitosan-0.4PBLO solution.

Conclusions
The present work reports the successful incorporation of Piper betle Linn oil in chitosan film (pCS-PBLO film) to produce potential active food packaging material. The microstructure of the pCS-PBLO film exhibited discontinuous and heterogeneous appear-

Conclusions
The present work reports the successful incorporation of Piper betle Linn oil in chitosan film (pCS-PBLO film) to produce potential active food packaging material. The microstructure of the pCS-PBLO film exhibited discontinuous and heterogeneous appearance by the presence of oil droplets on the film surface. Furthermore, the inter-molecular interaction among functional groups in chitosan and Piper betle Linn oil was confirmed by FTIR, XRD, and TGA analyses. The mechanical behavior and swelling degree were directly affected by the incorporation of PBLO. The pCS-PBLO film revealed the antibacterial and antioxidant activity based on phenolic compounds such as acetyleugenol, eugenol, 4-allyl-1,2-diacetoxybenzen, chavicol acetate in PBLO components; however, the bioactivity of resultant films was lower as compared to that in chitosan film containing Piper betle Linn extract in our previous report. Moreover, the great UV-barrier property and strong antioxidant activity was the light of the pCS-PBLO film. In particularly, the pCS-PBLO film may protect the shelf life of king oranges from the food deterioration for up to two weeks, suggesting that the film can be proposed for effective food packaging application.
Supplementary Materials: The following are available online at https://www.mdpi.com/2079-6 412/11/3/351/s1, Figure S1: Inhibitory effects of PBLLE incorporated chitosan films against the growth of Staphylococcus aureus, Salmonella Typhimurium, Escherichia coli, and Pseudomonas aeruginosa were observed via real photos taken after 24 h exposure, Figure S2: Inhibitory effects of PBLLE incorporated chitosan films against the growth of Escherichia coli was observed via real photos taken after 0 h, 4 h, 8 h, 11 h and 24 h exposure Table S1: Degradative temperature and mass loss of pCS, pCS-0.4PBLO, pCS-1PBLO, and pCS-1.2PBLO, Table S2: Surface tension, work of adhension, and spreading coefficient of chitosan solution with and without PBLO.

Conflicts of Interest:
The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper.